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A new look at kinetochore structure in vertebrate somatic cells using high-pressure freezing and freeze substitution

机译:利用高压冷冻和冷冻替代物对脊椎动物体细胞中线粒体结构的新认识

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摘要

Three decades of structural analysis have produced the view that the kinetochore in vertebrate cells is a disk-shaped structure composed of three distinct structural domains. The most prominent of these consists of a conspicuous electron opaque outer plate that is separated by a light-staining electron-translucent middle plate from an inner plate associated with the surface of the pericentric heterochromatin. Spindle microtubules terminate in the outer plate and, in their absence, a conspicuous corona of fine filaments radiates from the cytoplasmic surface of this plate. Here we report for the first time the ultrastructure of kinetochores in untreated and Colcemid-treated vertebrate somatic (PtK1) cells prepared for optimal structural preservation using high-pressure freezing and freeze substitution. In serial thin sections, and electron tomographic reconstructions, the kinetochore appears as a 50–75 nm thick mat of light-staining fibrous material that is directly connected with the more electron-opaque surface of the centromeric heterochromatin. This mat corresponds to the outer plate in conventional preparations, and is surrounded on its cytoplasmic surface by a conspicuous 100–150 nm wide zone that excludes ribosomes and other cytoplasmic components. High magnification views of this zone reveal that it contains a loose network of light-staining, thin (<9 nm diameter) fibers that are analogous to the corona fibers in conventional preparations. Unlike the chromosome arms, which appear uniformly electron opaque, the chromatin in the primary constriction appears mottled. Since the middle plate is not visible in these kinetochore preparations this feature is likely an artifact produced by extraction and coagulation during conventional fixation and/or dehydration procedures.
机译:三十年的结构分析得出这样的观点,脊椎动物细胞中的线粒体是由三个不同的结构域组成的盘状结构。其中最突出的是一个显眼的不透明电子外板,该板由光染色的电子半透明中间板与与周围同质异染色质表面相关的内板隔开。纺锤体微管终止于外板,在不存在时,显着的细丝日冕从该板的细胞质表面辐射出来。在这里,我们首次报告动植物超微结构在​​未经处理的和Colcemid处理的脊椎动物体细胞(PtK1)中的制备,以利用高压冷冻和冷冻替代获得最佳的结构保存。在连续的薄切片和电子断层扫描重建中,线粒体表现为厚度为50-75 nm的浅色纤维材料垫,直接与着丝粒异染色质的电子不透明表面直接连接。该垫子相当于常规制剂中的外板,在其细胞质表面上被一个明显的100-150 nm宽的区域包围,该区域不包括核糖体和其他细胞质成分。该区域的高倍放大图显示,该区域包含一个松散的浅色纤维网(直径小于9 nm),类似于常规制剂中的电晕纤维。与染色体臂均匀地呈现电子不透明不同,在初级颈缩中的染色质呈斑点状。由于在这些动线粒制剂中中间板是不可见的,因此该特征很可能是在常规固定和/或脱水程序中通过提取和凝结产生的伪影。

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